Enzymatic Decarboxylation of Tyrosine and Phenylalanine To

Purified tyrosine and phenylalanine were converted to tyramine and phenethylamine by tyrosine and phenylalanine decarboxylases, respectively...
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Anal. Chem. 2002, 74, 479-483

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Enzymatic Decarboxylation of Tyrosine and Phenylalanine To Enhance Volatility for High-Precision Isotopic Analysis Bassem I. Ziadeh,† Anthony L. Michaud,† Nabil M. R. Saad,† Betty A. Lewis,† Mahroukh Rafii,‡ Paul B. Pencharz,‡,§ and J. Thomas Brenna*,†

Division of Nutritional Sciences, Cornell University, Savage Hall, Ithaca, New York 14850, and The Research Institute, Hospital for Sick Children, and Department of Paediatrics and Nutritional Sciences, University of Toronto, Toronto, Ontario M5G 1X8, Canada

We present a rapid and selective method to increase the volatility of tyrosine and phenylalanine without adding derivative C for high-precision gas chromatographycontinuous-flow isotope ratio mass spectrometry (GCCIRMS) based on enzymatic decarboxylation to yield alkylamines and evaluated for 15N isotopic integrity. Purified tyrosine and phenylalanine were converted to tyramine and phenethylamine by tyrosine and phenylalanine decarboxylases, respectively. GC separation was achieved using a thick stationary phase (5-µm) capillary column. Recoveries were 95 ( 2%. The reproducibility of δ15N of tyramine and phenethylamine measured by GCC-IRMS averaged SD(δ15N) ) 0.33‰. The absolute differences between δ15N of amino acids measured by elemental analyzer-IRMS and the alkylamines measured by GCCIRMS was not significant. Phenethylamine and tyramine prepared from a mixture of 18 amino acids were extracted by ethanol with 95% recovery, and analysis yielded clean chromatograms and equivalent precision. These data indicate that enzymatic decarboxylation of phenylalanine and tyrosine is a convenient method to increase their volatility for continuous-flow isotopic analysis without introducing extraneous C or significant isotopic fractionation. Stable isotope tracer experiments using high-precision isotope ratio mass spectrometry (IRMS) are used extensively in many branches of biological research, including biochemistry, biomedicine, pharmacology, and ecology.1 Recent applications include the study of amino acid kinetics,2 assessment of amino acids requirement,3 measurement of plasma protein synthesis rate in humans,4,5 and 13C-based breath tests.6 * Corresponding author: (fax) (607) 255 1033; (phone) (607) 255 9128; (e-mail) [email protected]. † Cornell University. ‡ The Research Institute, Hospital for Sick Children, University of Toronto. § Department of Paediatrics and Nutritional Sciences, University of Toronto. (1) Goodman, K. J.; Brenna, J. T. Anal. Chem. 1992, 64, 1088-1095. (2) Fuller, M. F.; Garlick, P. J. Annu. Rev. Nutr. 1992, 14, 217-241. 10.1021/ac015558j CCC: $22.00 Published on Web 12/11/2001

© 2002 American Chemical Society

Isotopic measurement of 15N at high precision and around natural abundance has wide application in amino acid synthesis and metabolism studies.7-9 In enriched tracer applications, compound-specific isotopic analysis (CSIA) of 15N abundance by gas chromatography-continuous-flow isotope ratio mass spectrometry (GCC-IRMS) has been used to study the effect of the nonsteroidal antiinflammatory agent ibuprofen on the attenuation of the acute-phase response in colon cancer patients, utilizing 15N glycine as a tracer.10 15N-Labeled urea has been used as a tracer to show that Helicobactor pylori utilize urea as a source of nitrogen for synthesis of its amino acids.11 Three major challenges encountered in high-precision CSIA of 15N isotopic abundance, relative to C, have been outlined previously.12 First, the concentration of N compared to C in most organic compounds is low. For example, amino acids have 2-11 mol of C/mol of N. Second, for 15N/14N isotopic analysis, organic nitrogen must be reduced to N2, halving the analysis gas relative to CO2 used for C and resulting in a CO2/N2 ratio twice that of the sample C/N ratio. For the amino acids, the production of 1 mol equiv of N2 results in the formation of 4-22 mol equiv of C, without taking into consideration the carbon of the derivatizing reagent. Finally, the preponderance of N2 in ambient air translates (3) Zello, G. A.; Wykes, L. J.; Ball, R. O.; Pencharz, P. B. J. Nutr. 1995, 125, 2907-2915. (4) Velden M. G.; Rabelink, T. J.; Gadellaa, M. M.; Elzinga, H.; Reijngoud, D. J.; Kuipers, F.; Stellaard, F. Anal. Biochem. 1998, 265, 308-312. (5) Velden, M. G.; Kaysen, G. A.; de Meer, K.; Stellaard, F.; Voorbij, H. A.; Reijngoud, D. J.; Rabelink, T. J.; Koomans, H. A. Kidney Int. 1998, 53, 181-188. (6) Savarino, V.; Vigneri, S.; Celle, G. Gut 1999, 45 (Suppl. 1), I18-122. (7) Danicke, S.; Nieto, R.; Lobley, G. E.; Fuller, M. F.; Brown, D. S.; Milne, E.; Calder, A. G.; Chen, S.; Grant, I.; Bottcher, W. Arch. Tiererneahr. 1999, 52, 41-52. (8) Petzke, K. J.; Grigorov, J. G.; Korkushko, O. V.; Kovalenko, N. K.; Semesko, T. G.; Metges, C. C. Z. Ernaehrungswiss. 1998, 37, 368-375. (9) Gremaud, G.; Boza, J.; Piguet, C.; Duruz, E.; Acheson, K.; Ballevre, O.; Courtois, D. Isot. Environ. Health Stud. 1998, 34 (1-2), 148. (10) Preston, T.; Fearon, K. C.; McMillan, D. C.; Winstanley, F. P.; Slater, C.; Shenkin, A.; Carter, D. C. Br. J. Surg. 1995, 82, 229-234. (11) Williams, C. L.; Preston, T.; Hossack, M.; Slater, C.; McColl, K. E. FEMS Immunol. Med. Microbiol. 1996, 13, 87-94. (12) Augenstein, W. M. J. Chromatogr., A 1999, 842, 351-371.

Analytical Chemistry, Vol. 74, No. 2, January 15, 2002 479

into high N2 backgrounds even for small system leaks. These factors effectively increase sample size requirements. Matthews and Hayes13 first presented a system on-line separation of individual compounds for C and N isotopic measurements using a single collector instrument and calling their technique isotope ratio-monitoring gas chromatography-mass spectrometry (irmGCMS). Combustion converts most organic N into N2; the CO2 of combustion must be trapped at liquid N2 temperature to avoid co-introduction of CO2 into the ion source with N2; electron impact of CO2 creates CO+, which is an isobaric interference with N2 at m/z 28. In 1994, Preston and Slater reported a system with a conversion interface consisting of combustion furnace and liquid N2 cold trap to capture CO2 and H2O14 using a modern multicollector system. In the same year, Merritt and Hayes presented a similar system with the addition of a reduction furnace to convert residual nitrogen oxides to N2 for highest precision.15 Instruments for N-CSIA have been available for several years and are generally based on a combustion/reduction approach. Amino acids are usually derivatized prior to GC analysis and for continuous-flow 15N isotopic analysis to improve volatility and reduce H-bonding. Normal derivatization adds a number of moles of extraneous carbon to each mole of amino acid, the total number depending on the specific derivative group. Typical amounts of extraneous C are 5 mol of C/mol of amino acid for N-acetylisopropyl derivatives (NAP),16-19 5 mol of C/mol of amino acid for N-tert-butyldimethylsilyl-N-methyltrifluoracetamide (MTBSTFA) derivatives,20 and 8 mol of Cmol of amino acid for N-pivaloylisopropyl (NPP).17 While addition of extra C improves signal for GCflame ionization detection (FID), it poses problems for highprecision isotopic analysis. CO2 from derivative C cannot be distinguished from CO2 from the analyte; thus standards and correction factors must be applied for C analysis, as outlined previously.21 For N analysis, high CO2/N2 prematurely occludes cryotraps and degrades chromatographic performance. Ideally, the volatilization chemistry should introduce no extraneous C. We recently presented a general strategy for volatilization of nonpolar amino acids by chemical reduction with NaBH4 to yield amino alcohols.21 While this approach is potentially applicable to many more amino acids, the reactivity of chemical reagents produces complex product mixtures, often necessitating timeconsuming purification before or after the reaction. In contrast, enzyme-mediated reactions are highly specific for analyte or reaction and are usually less prone to catalyze side reactions. Enzymes have not been exploited as catalysts to alter analytes for high-precision isotopic analysis. In this paper, we demonstrate a strategy for increasing the volatility of tyrosine and phenylalanine by enzymatic decarboxylation to tyramine and phenethylamine. We present methods for decarboxylation and extraction of tyramine and phenethylamine (13) (14) (15) (16) (17) (18) (19) (20) (21)

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Mathews, D. E.; Hayes, J. M. Anal. Chem. 1978, 11, 1465-1473. Preston, T.; Slater, C. Proc. Nutr. Soc. 1994, 53, 363-372. Merrit, D. A.; Hayes, J. M. J. Am. Soc. Mass Spectrom. 1994, 5, 387-397. Metges, C. C.; Petzke, K. J.; Hennig, U. J. Mass Spectrom. 1996, 31, 367-376. Metges, C. C.; Petzke, K. J. Anal. Biochem. 1997, 247, 158-164. Yoneyama, T.; Fujihara, S.; Yagi, K. J. Exp. Bot. 1998, 320, 521-526. Yoneyama, T.; Tanaka, F. Soil Sci. Plant Nur. 1999, 45, 751-755. Hofmann, D.; Jung, K.; Bender, J.; Gehre, M.; Schuurmann, G. J. Mass Spectrom. 1997, 32, 855-863. Ziadeh, B. I.; Saad, N. M. R.; Lewis, B. A.; Brenna, J. T. Anal. Chem. 2001, 73, 799-802.

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from a mixture of 18 amino acids, show a GC method suitable for 15N isotopic analysis by continuous-flow GCC-IRMS, and evaluate possible isotopic fractionation by measuring the δ15N of amino acids by elemental analyzer (EA)-IRMS and their corresponding decarboxylated compounds. EXPERIMENTAL SECTION Amino Acids, Solvent, and Reagents. Purified and mixed amino acids were analytical grade, >98% purity, and obtained from Sigma Chemical Co. (St. Louis, MO). Sodium acetate, acetic acid, and ammonium hydroxide were obtained from Fisher Scientific Co. (Fair Lawn, NJ). Tyrosine decarboxylase and phenylalanine decarboxylase are derived from the bacteria Streptococcus faecalis, and their concentration is expressed in activity units, where 1 unit decarboxylates 1 µmol of tyrosine or phenylalanine per minute. Tyrosine decarboxylase (0.05 unit/mg of solid with excess pyridoxal 5-phosphate) and phenylalanine decarboxylase enzymes (from S. faecalis, 5 units/g) were obtained from Sigma Chemical Co. Decarboxylation of Tyrosine and Phenylalanine Standards. For evaluation of isotopic integrity by bulk analysis, purified tyrosine and phenylalanine standards were decarboxylated in separate experiments. Relatively large amounts were used because of the sample size requirements of bulk isotopic analysis, ∼1 mg of amino acid per determination, as detailed below. Tyrosine and phenylalanine were reacted according to procedures described previously22 with minor modifications. Tyrosine (100 mg) was dissolved in 50 mL of water with addition of 1 drop of 5 N NaOH to assist in solubilization. A 0.5-mL aliquot of this solution, 2 mg of tyrosine/mL (5.5 µM), was transferred to a small vial and the solvent was evaporated under nitrogen. Tyrosine decarboxylase (0.275 mg, equivalent to 0.01 unit), suspended in 0.1 M acetate buffer (2 mL, pH 5.5), was added and the mixture was shaken gently at 37 °C. After 3 h, the mixture was boiled to deactivate the enzyme and ultrafiltered (3000 MW cutoff) to remove protein; solvent was removed by evaporation. The sample was dissolved in 0.2 mL of water for analysis. Phenylalanine was decarboxylated according to procedures described previously22 with minor modifications. Phenylalanine (100 mg) was dissolved in 25 mL of water; 0.25 mL of the solution, equivalent to 1 mg (6 µmol), was transferred to a small vial, and the solvent was evaporated under nitrogen. Enzyme powder (165 mg), equivalent to 0.8 unit of phenylalanine decarboxylase, suspended in 0.1 M acetate buffer (2 mL, pH 5.5) was added to the vial, and the mixture was shaken gently at 37 °C for 3 h. The mixture was then boiled, utrafiltered, evaporated, and finally taken up in 0.2 mL of water. Decarboxylation of Phenylalanine and Tyrosine in a Mixture of 18 Amino Acids. A mixture of 18 amino acids in HCl (0.1 M, 1 mL, 2.5 µmol of each amino acid) was dried under nitrogen. Tyrosine decarboxylase and phenylalanine decarboxylase (2.5 units each) suspended in 0.1 M acetate buffer (2 mL, pH 5.5) at 37 °C were added to the mixture, which was then shaken gently for 3 h. Again the mixture was boiled, utrafiltered, and evaporated to dryness. The dried residue was extracted with 500 µL of 95% ethanol. The ethanol was evaporated, and (22) Battersby, A. R.; Chrystal, E. J.; Staunton, J. J. Chem. Soc., Perkin Trans. 1 1980, 1, 31-42.

the residue was taken up in water as a solvent for introduction to the GC. Yield and Purity of Tyramine and Phenethylamine. Aqueous solutions of tyramine and phenethylamine were injected into a HP 5890 GC equipped with a CP-sil 5CB fused-silica capillary column (50 m × 0.53 mm × 5 µm film thickness; Chrompack Inc.) with He carrier gas flow of 3.3 mL/min. Injection of 1 µL was performed using split mode 1:20. The oven temperature was isothermal at 250 °C. The injector and detector temperatures were 240 and 250 °C, respectively, for all GC analyses. Detection was by FID. Standard solutions of tyramine and phenethylamine were prepared to permit evaluation of GC-FID response, to allow calculation of yield. Preparation of Samples for Isotopic Analysis. An EA coupled to an IRMS was used to determine δ15N for nonvolatile tyrosine and phenylalanine standards. Histamine was used as a convenient isotopic standard because it is amenable to direct isotopic analysis by GCC-IRMS and EA-IRMS. Concentrated stock solutions were prepared for histamine, tyrosine, and phenylalanine to ensure isotopic homogeneity.23 From these solutions, samples of histamine, phenylalanine, and tyrosine containing 80 µg of total N for each were prepared for isotopic analysis in triplicate. A 20 µg/µL standard aqueous solution of histamine was transferred (10.6 µL) to tin capsules. For tyrosine, 520 µL of a 100 µg/50 µL standard solution in water was used, and for phenylalanine, 236 µL of 100 µg/25 µL aqueous solution was used. Water solvent was evaporated to dryness under nitrogen prior to EA analysis. Elemental analysis was performed using a Europa Scientific (Crewe, U.K.) ANCA elemental analyzer coupled to a model 20/20 IRMS. GCC-IRMS. The on-line isotopic analysis system consisted of a Varian GC (3400) coupled to a Europa Scientific 20/20 IRMS via an in-house-built combustion reactor/reduction reactor/water trap/liquid N2 cryogenic trap/open split interface. The GC was equipped with CP-sil 5CB fused-silica capillary column identical to that used for GC-FID analysis, as well as its own FID. By means of an automated two-position valve (Valco Instruments, Houston, TX) the analyte could be directed either to the FID for quantification and method development or to IRMS for isotopic analysis. The oven temperature was isothermal at 250 °C, and the injector and the detector temperatures were as before. The combustion furnace was made of 20 cm × 0.25 mm of deactivated fused silica filled with oxidized Cu wire surrounded by a heated ceramic furnace held at 850 °C. The reduction reactor was made of 20 cm × 0.25 mm deactivated fused silica filled with Cu wire surrounded by a heated ceramic furnace that was held at 550 °C. The water trap was of the Nafion type (DuPont, Wilmington, DE), which eliminates H2O while retaining CO2. The cryogenic trap consisted of a stainless steel capillary (30 cm × 1 mm i.d.), which passes through a Dewar filled with liquid nitrogen, and is connected upstream to the water trap exit and downstream to the open split. Separated analyte from the GC is swept into the combustion furnace by He carrier gas and quantitatively combusted into CO2, H2O, N2, and NxOy. The products pass into a reduction furnace, where NxOy are reduced to N2. (23) Caimi, R. J.; Houghton, L. A.; Brenna, J. T. Anal. Chem. 1994, 66, 29892991.

Figure 1. Chromatography of the extracted phenethylamine and tyramine from a mixture of 18 amino acids on CP-sil 5 CB fusedsilica capillary column (50 m × 0.53 mm; 5-µm film thickness) (Chrompack Inc.) with He carrier gas. The oven temperature was held at 250 °C.

One-microliter splitless injections were made of 2 µg/µL solutions of phenethylamine (16.6 nmol) and tyramine (14.5 nmol), containing 233 and 212 pmol of N2, respectively. About 7.7% of the analysis stream is admitted to the IRMS with the rest vented to atmosphere via the open split, representing a ∼13:1 split. RESULTS AND DISCUSSION Decarboxylation and Chromatography. Alkylamines that are produced by decarboxylation of the amino acids are strongly H-bonding analytes, which tend to interact with the walls of the fused-silica capillary column when analyzed with a conventional 0.25-µm film capillary column. To avoid tailing, we used the same strategy as reported previously21 to analyze amino alcohols. A thick stationary phase (5 µm) masks analyte from the capillary column walls when analyte loads well below column capacity are injected. Decarboxylation of purified phenylalanine or tyrosine produces clean chromatograms with no evidence of any contaminants (data not shown). Comparison of peak areas with standards demonstrates a yield of 95 ( 2% for these 3-h reaction times. Figure 1 shows the chromatogram of the decarboxylated products phenethylamine and tyramine, isolated from a mixture of 18 amino acids after enzymatic decarboxylation. Sharp peaks are obtained with no evidence of extraneous peaks reflective of stray reagents or unreacted materials. Chromatograms such these are compatible with GC introduction to IRMS for isotopic analysis and are ideal for quantitative analysis as well. Yields from the mixture were 95 ( 2%, as for the purified standards. The results of the nitrogen isotopic analyses of the alkylamines measured by GCC-IRMS and of the amino acids measured by EA-IRMS are presented in Table 1. Tyrosine and phenylalanine averaged δ15Nair ) 8.02‰ and 1.03‰, respectively, while tyramine and phenethylamine averaged δ15Nair ) 8.28‰ and 1.49‰, respectively. The analytical error obtained from replicates of amino acids analyzed by EA-IRMS averaged SD(δ15N) ) 0.35‰, while the average error of the alkylamine replicates measured by GCCIRMS was SD(δ15N)) 0.31‰. The difference between δ15N of the EA analysis of the amino acid and δ15N of the GCC-IRMS analysis of the corresponding alkylamines shown in Table 1 averaged ∆δ15N ) -0.36‰, and they were not statistically significant (p